Custom made inclusion bodies: impact of classical process parameters and physiological parameters on inclusion body quality attributes

Christoph Slouka; Julian Kopp; Stefan Hutwimmer; Michael Strahammer; Daniel Strohmer; Elisabeth Eitenberger; Andreas Schwaighofer; Christoph Herwig

doi:10.1186/s12934-018-0997-5

Custom made inclusion bodies: impact of classical process parameters and physiological parameters on inclusion body quality attributes

Microb Cell Fact. 2018 Sep 20;17(1):148. doi: 10.1186/s12934-018-0997-5.

Authors

Christoph Slouka¹, Julian Kopp¹, Stefan Hutwimmer², Michael Strahammer¹, Daniel Strohmer¹, Elisabeth Eitenberger³, Andreas Schwaighofer³, Christoph Herwig^{4

5}

Affiliations

¹ Christian Doppler Laboratory for Mechanistic and Physiological Methods for Improved Bioprocesses, Institute of Chemical Engineering, Vienna University of Technology, Vienna, Austria.
² Sandoz GmbH, Biochemiestrasse 10, 6250, Kundl, Tirol, Austria.
³ Institute of Chemical Technology and Analytics, Getreidemarkt 9/164, 1060, Vienna, Austria.
⁴ Christian Doppler Laboratory for Mechanistic and Physiological Methods for Improved Bioprocesses, Institute of Chemical Engineering, Vienna University of Technology, Vienna, Austria. christoph.herwig@tuwien.ac.at.
⁵ Institute of Chemical, Environmental and Bioscience Engineering, Research Area Biochemical Engineering, Vienna University of Technology, Gumpendorfer Strasse 1a, 1060, Vienna, Austria. christoph.herwig@tuwien.ac.at.

Abstract

Background: The bacterium E. coli is a major host for recombinant protein production of non-glycosylated products. Depending on the expression strategy, the recombinant protein can be located intracellularly. In many cases the formation of inclusion bodies (IBs), protein aggregates inside of the cytoplasm of the cell, is favored in order to achieve high productivities and to cope with toxic products. However, subsequent downstream processing, including homogenization of the cells, centrifugation or solubilization of the IBs, is prone to variable process performance or can be characterized by low extraction yields as published elsewhere. It is hypothesized that variations in IB quality attributes (QA) are responsible for those effects and that such attributes can be controlled by upstream process conditions. This contribution is aimed at analyzing how standard process parameters, such as pH and temperature (T) as well as different controlled levels of physiological parameters, such as specific substrate uptake rates, can vary IB quality attributes.

Results: Classical process parameters like pH and T influence the expression of analyzed IB. The effect on the three QAs titer, size and purity could be successfully revealed. The developed data driven model showed that low temperatures and low pH are favorable for the expression of the two tested industrially relevant proteins. Based on this knowledge, physiological control using specific substrate feeding rate (of glucose) q_s,Glu is altered and the impact is tested for one protein.

Conclusions: Time dependent monitoring of IB QA-titer, purity, IB bead size-showed a dependence on classical process parameters pH and temperature. These findings are confirmed using a second industrially relevant strain. Optimized process conditions for pH and temperature were used to determine dependence on the physiological parameters, the specific substrate uptake rate (q_s,Glu). Higher q_s,Glu were shown to have a strong influence on the analyzed IB QAs and drastically increase the titer and purity in early time stages. We therefore present a novel approach to modulate-time dependently-quality attributes in upstream processing to enable robust downstream processing.

Keywords: Escherichia coli; Inclusion body quality attributes; Recombinant protein production; Upstream development.

MeSH terms

Cytoplasm / metabolism
Escherichia coli*
Hydrogen-Ion Concentration
Inclusion Bodies / metabolism*
Metabolic Engineering / methods
Protein Aggregates
Recombinant Proteins / biosynthesis
Temperature

Substances

Protein Aggregates
Recombinant Proteins